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确定性单细胞RNA测序可捕捉肠道隐窝和类器官组成的变化。

Deterministic scRNA-seq captures variation in intestinal crypt and organoid composition.

作者信息

Bues Johannes, Biočanin Marjan, Pezoldt Joern, Dainese Riccardo, Chrisnandy Antonius, Rezakhani Saba, Saelens Wouter, Gardeux Vincent, Gupta Revant, Sarkis Rita, Russeil Julie, Saeys Yvan, Amstad Esther, Claassen Manfred, Lutolf Matthias P, Deplancke Bart

机构信息

Laboratory of Systems Biology and Genetics, Institute of Bioengineering, School of Life Sciences, École Polytechnique Fédérale de Lausanne (EPFL), Lausanne, Switzerland.

Swiss Institute of Bioinformatics (SIB), Lausanne, Switzerland.

出版信息

Nat Methods. 2022 Mar;19(3):323-330. doi: 10.1038/s41592-021-01391-1. Epub 2022 Feb 14.

Abstract

Single-cell RNA sequencing (scRNA-seq) approaches have transformed our ability to resolve cellular properties across systems, but are currently tailored toward large cell inputs (>1,000 cells). This renders them inefficient and costly when processing small, individual tissue samples, a problem that tends to be resolved by loading bulk samples, yielding confounded mosaic cell population read-outs. Here, we developed a deterministic, mRNA-capture bead and cell co-encapsulation dropleting system, DisCo, aimed at processing low-input samples (<500 cells). We demonstrate that DisCo enables precise particle and cell positioning and droplet sorting control through combined machine-vision and multilayer microfluidics, enabling continuous processing of low-input single-cell suspensions at high capture efficiency (>70%) and at speeds up to 350 cells per hour. To underscore DisCo's unique capabilities, we analyzed 31 individual intestinal organoids at varying developmental stages. This revealed extensive organoid heterogeneity, identifying distinct subtypes including a regenerative fetal-like Ly6a stem cell population that persists as symmetrical cysts, or spheroids, even under differentiation conditions, and an uncharacterized 'gobloid' subtype consisting predominantly of precursor and mature (Muc2) goblet cells. To complement this dataset and to demonstrate DisCo's capacity to process low-input, in vivo-derived tissues, we also analyzed individual mouse intestinal crypts. This revealed the existence of crypts with a compositional similarity to spheroids, which consisted predominantly of regenerative stem cells, suggesting the existence of regenerating crypts in the homeostatic intestine. These findings demonstrate the unique power of DisCo in providing high-resolution snapshots of cellular heterogeneity in small, individual tissues.

摘要

单细胞RNA测序(scRNA-seq)方法已经改变了我们解析跨系统细胞特性的能力,但目前这些方法是针对大量细胞输入(>1000个细胞)设计的。当处理小的单个组织样本时,这使得它们效率低下且成本高昂,这个问题通常通过加载批量样本解决,从而产生混淆的镶嵌细胞群体读数。在这里,我们开发了一种确定性的、mRNA捕获珠和细胞共封装液滴系统DisCo,旨在处理低输入样本(<500个细胞)。我们证明,DisCo通过结合机器视觉和多层微流体技术,实现了精确的颗粒和细胞定位以及液滴分选控制,能够以高捕获效率(>70%)和每小时高达350个细胞的速度连续处理低输入单细胞悬液。为了强调DisCo的独特能力,我们分析了31个处于不同发育阶段的单个肠类器官。这揭示了广泛的类器官异质性,识别出不同的亚型,包括一种再生性的胎儿样Ly6a干细胞群体,即使在分化条件下也以对称囊肿或球体的形式持续存在,以及一种主要由前体和成熟(Muc2)杯状细胞组成的未表征的“杯状样”亚型。为了补充这个数据集并证明DisCo处理低输入、体内来源组织的能力,我们还分析了单个小鼠肠隐窝。这揭示了存在与球体组成相似的隐窝,其主要由再生干细胞组成,表明在稳态肠道中存在再生隐窝。这些发现证明了DisCo在提供小的单个组织中细胞异质性的高分辨率快照方面的独特能力。

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